Search
Menu
Optimax Systems, Inc. - Ultrafast Coatings 2024 LB

Graphene Properties Add Axial Resolution Precision to 3D Imaging

Facebook X LinkedIn Email
MUNICH, March 14, 2023 — Researchers at the Ludwig Maximilian University of Munich (LMU) combined pulsed-interleaved MINFLUX (pMINFLUX) nanoscopy with a newly developed method for axial resolution that exploits the special properties of the 2D material graphene to achieve 3D, superresolution imaging with nanometer-scale precision. The researchers combined the 2D localization of pMINFLUX with axial information from graphene energy transfer (GET) and with single-molecule switching using DNA point accumulation for imaging in nanoscale topography (DNA-PAINT).

DNA-PAINT is a single-molecule localization microscopy technique that supports multiplexed imaging of fluorescently tagged molecules at high spatial resolution.

Using this approach, the team achieved a localization precision in 3D of less than 2 nm, with axial precision below 0.3 nm. By achieving molecular and even submolecular resolution, 3D superresolution microscopy with nanometer precision will enable new insights into nanostructures and biological systems. The synergetic combination of pMINFLUX and GET allows for superresolution imaging near the surface, for investigating cell adhesion and membrane complexes, for example.

pMINFLUX was introduced by the LMU lab in 2020 as a simplified version of MINFLUX (minimal photon FLUX), a superresolution imaging method that itself combines aspects of single-molecule localization microscopy and stimulated emissions depletion microscopy. In addition to being simpler than the method on which it is built, pMINFLUX also provides the fluorescence lifetime.

MINFLUX interrogates the location of each molecule by focusing a laser near the molecule and measuring the molecule’s distance from the center of the laser focus according to the fluorescence intensity. Researchers can obtain the exact position of the molecule by placing the center of the laser focus at different, successive positions in relation to the molecule.

When pMINFLUX and GET are combined, the information of each photon can be synergistically used for both 2D and axial localization information. Binding sites are placed precisely in 3D by using DNA origami nanopositioners, fluorescent molecules, and DNA-PAINT. The nanopositioners are then used to evaluate the combination of GET, pMINFLUX, and DNA-PAINT for 3D localization and 3D superresolution imaging at different distances from the graphene.

Due to the use of GET, the fluorescence lifetime is distance-dependent; therefore, a change in the fluorescence lifetime can be converted to axial distance from graphene.

This enables GET-pMINFLUX to provide 3D localization with an axial precision of less than 3 Å.

“With the combination of pMINFLUX and graphene, the information of a photon is used in the best possible way,” professor Philip Tinnefeld said. “Here, pMINFLUX is synergistically combined with graphene energy transfer (GET) to enable precisions so far unreached for fluorescence microscopy.”
(a): pMINFLUX interrogates the position of a fluorophore with multiple spatially displaced doughnut beams and yields 2D fluorescence lifetime images with nm precision. (b): Graphene provides a measure for the axial distance to graphene. The fluorescence lifetime shortens the closer a fluorophore is to graphene. (c): Combining the lateral information of pMINFLUX with the axial graphene distance information yields 3D localizations. GET-pMINFLUX yields photon-efficient localizations with nm precision. This enables L-PAINT. The schematic of the DNA origami structure has a DNA-pointer protruding. this dense structure is localized within 2 s with nm precision and in 3D by combining L-PAINT and GET-pMINFLUX. Courtesy of J. Zähringer, F. Cole, et al.
(a) pMINFLUX interrogates the position of a fluorophore with multiple spatially displaced doughnut beams and yields 2D fluorescence lifetime images with nanometer precision. (b) Graphene provides a measure for the axial distance to graphene. The fluorescence lifetime shortens the closer a fluorophore is to graphene. (c) Combining the lateral information of pMINFLUX with the axial graphene distance information yields 3D localizations. GET-pMINFLUX yields photon-efficient localizations with nanometer precision. This enables L-PAINT. The schematic of the DNA origami structure has a DNA-pointer protruding. This dense structure is localized within 2 s with nanometer precision and in 3D by combining L-PAINT and GET-pMINFLUX. Courtesy of Light: Science and Applications (2023) DOI: 10.1038/s41377-023-01111-8.
pMINFLUX yields ultrahigh localization precision in xy; GET synergistically provides z-localization close to the coverslip surface, enabled by the fluorescence lifetime information of pMINFLUX; and DNA-PAINT provides the switching mechanism to proceed from superlocalization to superresolution. These three complementary components make comprehensive use of the information of each photon that is detected. According to the researchers, each component can be realized somewhat easily.

PFG Precision Optics - Precision Optics 12/24 MR

“The high precisions achievable with GET-pMINFLUX enable the development of methodologically new approaches to improve superresolution microscopy which were previously not realizable,” researcher Jonas Zähringer said. “Typically, the entire photon budget of a dye is needed to localize a position with 1-nm precision. However, GET-pMINFLUX is so photon-efficient that the photon budget can be split among multiple positions and still yield nanometer-precise localizations.”

To overcome the comparatively small field of view of pMINFLUX and the limited binding kinetics of DNA-PAINT, the researchers developed local PAINT (L-PAINT) using DNA nanotechnology. In contrast to DNA-PAINT, which enables superresolution by binding and unbinding a DNA strand labeled with fluorescent dye, L-PAINT has two binding sequences. The researchers designed a binding hierarchy in which the L-PAINT DNA strand binds for longer times on one side. This allows the other end of the strand to scan for binding sites with a high local concentration. The researchers demonstrated L-PAINT by imaging a triangular structure with 6-nm side lengths within seconds.

“The combination with GET-pMINFLUX and L-PAINT allows us to study structures and dynamics at the molecular level, which are fundamental for our understanding of cellular biomolecular reactions,” Tinnefeld said.

In the future, GET-pMINFLUX nanoscopy could be used to investigate artificial bilayers, cellular membranes, and adhesion complexes, as well as macromolecular complexes, with nanometer-scale, 3D precision.

The research was published in Light: Science & Applications (www.doi.org/10.1038/s41377-023-01111-8).

Published: March 2023
Glossary
superresolution
Superresolution refers to the enhancement or improvement of the spatial resolution beyond the conventional limits imposed by the diffraction of light. In the context of imaging, it is a set of techniques and algorithms that aim to achieve higher resolution images than what is traditionally possible using standard imaging systems. In conventional optical microscopy, the resolution is limited by the diffraction of light, a phenomenon described by Ernst Abbe's diffraction limit. This limit sets a...
fluorescence
Fluorescence is a type of luminescence, which is the emission of light by a substance that has absorbed light or other electromagnetic radiation. Specifically, fluorescence involves the absorption of light at one wavelength and the subsequent re-emission of light at a longer wavelength. The emitted light occurs almost instantaneously and ceases when the excitation light source is removed. Key characteristics of fluorescence include: Excitation and emission wavelengths: Fluorescent materials...
Imagingmolecularmolecular imagingMicroscopysuperresolutionsuperresolution 3-D imagingsuperresolution microscopysuperresolution microscope systemmultimodalmultimodal imagingfluorescencefluorescence imagingResearch & TechnologyeducationEuropeLudwig Maximilian UniversityDNA origamiaxialnanoscopychemical

We use cookies to improve user experience and analyze our website traffic as stated in our Privacy Policy. By using this website, you agree to the use of cookies unless you have disabled them.